Use of DNA sequence and mutant analyses and antisense oligodeoxynucleotides to examine the molecular basis of nonmuscle myosin light chain kinase autoinhibition, calmodulin recognition, and activity.

Shoemaker, M O; Lau, W.; Shattuck, R L; Kwiatkowski, A; Matrisian, P E; Guerra-Santos, L.; Wilson, Erica; Lukas, Thomas J.; Eldik, Linda J. Van; Watterson, Daniel

doi:10.1083/jcb.111.3.1107

Cited by 165 publications

(127 citation statements)

References 82 publications

Supporting

Mentioning

114

Contrasting

Order By: Relevance

“…The removal of the calmodulin regulatory domain (DCaM mutant) generated a constitutively active kinase (i.e., a gain of function mutation). This is consistent with previous information on other well studied calmodulin-dependent kinases, in which the calmodulin-regulatory domain has inhibitory e ects on the kinase activity, relieved by binding to Ca 2+ / calmodulin (Shoemaker et al, 1990). DAP-kinase activity was abolished by the substitution of a conserved lysine by alanine residue within the kinase domain (K42A), thus generating an inactive kinase mutant with potential dominant-negative activity .…”

Section: Biochemistry Of Dap-kinasesupporting

confidence: 91%

Death associated proteins (DAPs): from gene identification to the analysis of their apoptotic and tumor suppressive functions

1998

View full text Add to dashboard Cite

The process of apoptosis (programmed cell death) has become the subject of intensive and extensive research over the past few years. Various approaches are being used to identify and study genes which function as positive mediators of apoptosis. Here, we address a novel approach of gene cloning aimed at isolating intracellular death promoting genes by utilizing a functional screen. This method, called TKO, was based on transfection of cells with an anti-sense cDNA library, followed by the selection of transfectants which survived in the continuous presence of a killing cytokine ± interferon-g. It led to the identi®cation of ®ve novel apoptotic genes and to the ®nding that a known protease ± cathepsin D, is actively recruited to the death process. The ®ve novel apoptotic genes (named DAP genes for: Death Associated Proteins) code for proteins which display a diverse spectrum of biochemical activities. The list comprises a novel type of calcium/calmodulin-regulated kinase which carries ankyrin repeats and a death domain (DAPkinase), a nucleotide-binding protein (DAP-3), a small proline-rich cytoplasmic protein (DAP-1), and a novel homolog of the eIF4G translation initiation factor (DAP-5). Extensive studies proved that these genes are critical for mediating cell death initiated by interferon-g, and in some of the tested cases also cell death induced by Fas/APO-1, TNF-a, and a detachment from extracellular matrix. Moreover, one of these genes, DAP-kinase, was recently found to display strong tumor suppressive activities, coupling the control of apoptosis to metastasis.The advantage of functional approaches of gene cloning is that they select the relevant rate limiting genes along the death pathways in a complete unbiased manner. As a consequence, novel targets and unpredicted mechanisms emerged. A few examples illustrating this important point will be discussed. One relates to the calcium/calmodulin-dependent DAP-kinase, which is localized to the actin micro®laments. It was found that the correct localization of DAP-kinase to the micro®la-ment network was critical for the execution of the apoptotic process, and more speci®cally for the disruption of the stress ®bers ± a typical hallmark of apoptosis. Another important breakthrough step in our understanding of apoptotic processes relates to the identi®ca-tion and analysis of the DAP-5 gene. The structure/ function features of this novel translation regulator resemble the proteolytically cleaved eIF4G which appears in cells upon infection with some RNA viruses and which directs cap-independent translation. Thus, the rescue of DAP-5 highlighted the importance of regulation of protein translation in certain apoptotic systems. Finally, the isolation of cathespin D by our method suggests that lysosomal proteases are recruited during apoptosis, in addition to the well known caspase family of proteases, and that a unique pattern of regulation a ecting the processing of this protease takes place. The major challenge now is to analyse how these diverse DAP gene activities co...

show abstract

Section: Biochemistry Of Dap-kinasesupporting

confidence: 91%

Death associated proteins (DAPs): from gene identification to the analysis of their apoptotic and tumor suppressive functions

1998

View full text Add to dashboard Cite

show abstract

“…A double charge cluster reversal mutation where D l 18-El20 was also replaced by KKK yielded almost no activation of sk-MLCK (Weber et al, 1989). Shoemaker et al (1990) showed that for fibroblast MLCK (CaM binding sequence identical to sm-MLCK), the K, for the substrate peptide was higher in the presence of E84K or E120K mutant CaMs, but decreased to the same value as the wild type if a charge reversa1 RRK-EEE was introduced at the beginning of the CaM binding region. In the crystal structure of CaM with the sm-MLCK peptide, both E120 and El 14 in the C-domain interact with basic residues in the N-terminal region of the peptide (Meador et al, 1992).…”

Section: Discussionmentioning

confidence: 99%

Role of the N‐terminal region of the skeletal muscle myosin light chain kinase target sequence in its interaction with calmodulin

Findlay¹,

Gradwell²,

Bayley³

1995

Protein Science

View full text Add to dashboard Cite

show abstract

“…EC MLCK-1 exhibited substantial time-dependent p60 src -catalyzed incorporation of radioactive phosphate (Fig. 2), whereas p60 src -mediated 32 P incorporation did not occur in either MLCK-2, the EC MLCK splice variant, lacking the 69-amino acid stretch containing the p60 src consensus site, nor in SM MLCK, which completely lacks the novel N terminus (Fig. 2).…”

Section: In Vitro Phosphorylation Of Mlck Isoforms By P60mentioning

confidence: 99%

“…Phosphorylation of MLCK diluted in reaction buffer was started by adding 0.2 mM ATP, 10 Ci/ml [␥- 32 P]ATP and 75 units/ml recombinant p60 src kinase (Upstate Biotechnology, Inc., Lake Placid, NY; final concentrations). Synthetic MLCK-1 peptides were used for p60 src phosphorylation assays at 0.1 mg/ml final concentration.…”

Section: Phosphorylation Of Mlck By P60 Src In Vitromentioning

confidence: 99%

Differential Regulation of Alternatively Spliced Endothelial Cell Myosin Light Chain Kinase Isoforms by p60Src

Birukov

Csortos

Marzilli

et al. 2001

Journal of Biological Chemistry

146

136

View full text Add to dashboard Cite

The Ca 2؉ /calmodulin-dependent endothelial cell myosin light chain kinase (MLCK) triggers actomyosin contraction essential for vascular barrier regulation and leukocyte diapedesis. Two high molecular weight MLCK splice variants, EC MLCK-1 and EC MLCK-2 (210 -214 kDa), in human endothelium are identical except for a deleted single exon in MLCK-2 encoding a 69-amino acid stretch ( 20 by Ca 2ϩ /calmodulin-dependent enzyme MLCK is essential for the initiation of nonmuscle and smooth muscle contraction (1, 3, 9 -11). In specific nonmuscle tissues, such as the vascular endothelium, this kinase is known to be involved in endothelial cell migration, cell retraction (12), endothelial cell barrier regulation (13), transendothelial migration of neutrophils (14, 15), and possibly apoptosis (16). The MLCK isoform abundantly expressed in smooth muscle (SM MLCK) generally exists as a 130-to 150-kDa protein that has been well characterized (for review see Refs. 3 and 11). However, Western blot screening of a variety of embryonic and adult smooth muscle and nonmuscle tissues revealed expression of a high molecular weight MLCK variant with electrophoretic mobility in the range of [208][209][210][211][212][213][214]. Garcia and colleagues (20) subsequently sequenced the high molecular weight MLCK isoform cloned from a human endothelial cell cDNA library, revealing an open reading frame, which encodes a protein of 1914 amino acids. Both the low molecular mass (130 -150 kDa) and high molecular mass (208 -214 kDa) MLCK isoforms share essentially identical actin binding, MLC binding, catalytic, and Ca 2ϩ /CaM-regulatory domains. The extreme C-terminal kinase-related protein (KRP) domain, which binds myosin, is contained within both EC MLCK and SM MLCK but can be also expressed as an independent protein capable of stabilizing myofilaments in vitro (3,(21)(22)(23). The C-terminal half of the endothelial MLCK isoform (residues 923-1914) exhibits 99.8% homology to the human low molecular weight MLCK from hippocampus and substantial homology to published SM MLCK sequences from rabbit (94% homology), bovine (95% homology), and chicken (85% homology) (5, 6, 24, 25). However, the exact biological function of the 922-amino acid N-terminal portion, which is unique to the high

show abstract

Use of DNA sequence and mutant analyses and antisense oligodeoxynucleotides to examine the molecular basis of nonmuscle myosin light chain kinase autoinhibition, calmodulin recognition, and activity.

Cited by 165 publications

References 82 publications

Death associated proteins (DAPs): from gene identification to the analysis of their apoptotic and tumor suppressive functions

Death associated proteins (DAPs): from gene identification to the analysis of their apoptotic and tumor suppressive functions

Role of the N‐terminal region of the skeletal muscle myosin light chain kinase target sequence in its interaction with calmodulin

Differential Regulation of Alternatively Spliced Endothelial Cell Myosin Light Chain Kinase Isoforms by p60Src

Contact Info

Product

Resources

About